Abstract

Background

The microbiota of the bovine upper respiratory tract has been recently characterized, but no data for the lower respiratory tract are available. A major health problem in bovine medicine is infectious bronchopneumonia, the most common respiratory syndrome affecting cattle. With this study, we used 16S rRNA gene sequencing to characterize and compare the microbial community composition of the upper and lower respiratory tracts in calves.

Results

The microbiota of the upper (nasal swab [NS]) and the lower (trans-tracheal aspiration [TTA]) respiratory tracts of 19 post-weaned Piedmontese calves with (8/19) and without (11/19) clinical signs of respiratory disease, coming from six different farms, was characterized by 16S rRNA gene metabarcoding. A total of 29 phyla (29 in NS, 21 in TTA) and 305 genera (289 in NS, 182 in TTA) were identified. Mycoplasma (60.8%) was the most abundant genus identified in both the NS (27.3%) and TTA (76.7%) samples, followed by Moraxella (16.6%) in the NS and Pasteurella (7.3%) in the TTA samples. Pasteurella multocida (7.3% of total operational taxonomic units [OTUs]) was the most abundant species in the TTA and Psychrobacter sanguinis (1.1% of total OTUs) in the NS samples. Statistically significant differences between the NS and the TTA samples were found for both alpha (Shannon index, observed species, Chao1 index, and Simpson index; P = 0.001) and beta (Adonis; P = 0.001) diversity. Comparison of the NS and TTA samples by farm origin and clinical signs revealed no statistical difference (P > 0.05), except for farm origin for the NS samples when compared by the unweighted UniFrac metric (P = 0.05).

Conclusions

Using 16S rRNA gene sequencing, we characterized the microbiota of the upper and lower respiratory tracts of calves, both healthy individuals and those with clinical signs of respiratory disease. Our results suggest that environmental factors may influence the composition of the upper airway microbiota in cattle. While the two microbial communities (upper and lower airways) differed in microbial composition, they shared several OTUs, suggesting that the lung microbiota may be a self-sustaining, more homogeneous ecosystem, influenced by the upper respiratory tract microbiota.

Background

In the last decade, the use of high-throughput sequencing methods (next-generation sequencing, NGS) coupled to DNA barcoding has advanced the study of bacterial communities as a whole [1]. DNA metabarcoding allows the generation of multiple reads of the hypervariable regions of the 16S rRNA gene in a single run, thus yielding a wealth of phylogenetic information in a single experiment [1]. The 16S rRNA gene metabarcoding approach applied to lower respiratory tract samples from humans led to the discovery that the lung is not sterile even in healthy conditions [2]. The finding of lung microbiota in a healthy subject was initially explained as a temporal contamination from the upper respiratory tract either during sampling or by microaspiration [3]. However, recent studies have shown that the microbiota of the lung could be considered an ecosystem and that its composition depends on the immigration, elimination, and reproduction rates of the microbial communities present there [4,5,6]. Though the components of this ecosystem derive from the upper respiratory tract, they could be able to proliferate in the lungs and form a self-sustaining lung microbiota [4,5,6]. DNA metabarcoding analysis of pathological respiratory samples led to the hypothesis that alteration of the lung microbiota could assume a key role in the pathogenesis of human lung diseases, including bacterial pneumonia [6, 7].

Study of the bovine respiratory tract holds huge importance because one of the main health issues in the cattle industry is infectious bronchopneumonia, defined as bovine respiratory disease (BRD) [8, 9]. In Europe, BRD is associated with high morbidity and mortality, which leads to a widespread use of antimicrobials and, therefore, increases the alarm about antibiotic resistance [10,11,12,13,14,15,16,17,18,19]. BRD is a multifactorial disease resulting from interactions between management, physiologic, and environmental factors and etiological agents [20, 21]. The bacterial pathogens most often identified by culture-based methods in the course of BRD are Mannheimia haemolytica, Pasteurella multocida, Histophilus somni, and Mycoplasma bovis [22]. Considered ubiquitous inhabitants of the bovine upper respiratory tract, these bacterial species can proliferate in the lungs when inhaled during stressful events or viral infections [22]. However, they have also been isolated from the lower respiratory tract of calves not presenting clinical signs, raising questions about their role in the development of BRD [23, 24]. A better understanding of the etiology of BRD is critical to improve animal health.

In cattle, 16S rRNA gene metabarcoding to characterize the microbiota of the upper respiratory tract has been applied on nasal swab samples from dairy and beef calves [25,26,27,28,29,30,31]. Timsit et al. [26] and Holman et al. [28], for example, reported that the upper respiratory tract microbiota of beef cattle is not stable in the first 40 days on feedlot, possibly explaining their higher susceptibility for developing BRD in this period. Moreover, Lima et al. [31] found that the upper respiratory tract microbiota of dairy calves significantly differed depending on the animal’s clinical respiratory status. The application of this new technique to respiratory tract samples has attracted increasing interest; however, to our knowledge, data about the bovine lower respiratory tract microbiota are still lacking. The goal of this study was to characterize the microbiota of the upper and lower respiratory tracts by applying 16S rRNA gene metabarcoding on nasal swab (NS) and trans-tracheal aspiration (TTA) samples from post-weaned Piedmontese calves with and without clinical signs of BRD.

Methods

Sample population and sample collection

The study was performed in Piedmont, northwest Italy. The six farms included in the study were located in the provinces of Torino (TO), Cuneo (CN), and Vercelli (VC). The median distance as the crow flies between the farms was 50 km (min-max, 11–97 km) (map given in Additional file 1). The six farms were located in a restricted area with similar geographical and climatic characteristics. The farms were all cow-calf operations with the same animal management. Briefly, the calves were held with the mother until the end of the weaning period (5 months), then moved to multiple straw-bedded boxes (5–10 animals) with free access to water and feed (roughage and concentrate).

The animals included were post-weaned Piedmontese calves receiving veterinary care by the Veterinary Teaching Hospital of the University of Turin. Medical history and physical examination data were collected via a standardized collection form for each calf. A complete physical examination was performed for all animals focusing on typical clinical signs of BRD: cough, nasal discharge, and abnormal sounds at thoracic auscultation (wheezes, crackles) (Master Classic II™, 3M Littmann® stethoscope, 3M, St. Paul, MN, USA). Calves that had been treated in the week prior to examination or presented clinical signs suggestive of diseases different from BRD were excluded from the study.

Nasal swab (NS) samples were collected using sterile swabs (17 cm, DrySwab, Copan S.p.A, Italy) from both nostrils of each calf after cleaning the nostrils with 90% ethyl alcohol. Trans-tracheal aspiration (TTA) was performed as previously described [23]. Briefly, the animals were mildly sedated with intravenous injection of 0.05 mg/kg Xylasine (Rompun®, Bayer Healthcare, Germany), and an area of 3 × 3 cm about 7–10 cm caudal to the larynx was shaved and surgically prepared with 90% ethyl alcohol and iodophors. The area was desensitized with 4% procaine hydrochloride (Aticain®, A.T.I., Italy), and a longitudinal 1-cm incision was then placed in the midline directly above the trachea. A 12-G needle was used to perforate the trachea between two cartilage rings. A male dog urinary catheter (2 mm × 50 cm; Buster, sterile dog catheter, Kruuse, Germany) was introduced into the needle and pushed down into the airway for about 45 cm. Finally, a volume of 50 ml sterile 0.9% saline solution was injected through the catheter and immediately aspirated. To prevent sample contamination, a new sterile kit and a new pair of sterile gloves were used for each calf. All samples were stored at − 80 °C until analysis.

DNA extraction and library preparation

DNA extraction

DNA was isolated using DNAzol® reagent (Invitrogen, Carlsbad, CA, USA) according to the manufacturer’s instructions. Briefly, the NS were dipped in 500 μl of DNAzol® reagent immediately after collection, while the TTA fluids were pelleted and added with 1 ml of DNAzol® reagent, after thawing at 4 °C. The samples were then repeatedly homogenized and incubated at 4 °C for 18 h. After DNA precipitation by means of ethanol, the pellets were rinsed twice. Finally, DNA was eluted in 30 μl of RNase and DNase free water. The DNA concentration of each sample was determined using a Qubit fluorimeter (Qubit®, Invitrogen) and normalized to 5 ng/μl. Samples with a lower DNA concentration were not processed further.

Library preparation

The normalized DNA was processed according to the 16S Metagenomic Sequencing Library Preparation protocol as recommended by Illumina (Illumina, San Diego, CA, USA). Briefly, 12.5 ng of genomic DNA underwent an initial PCR step with the 16S amplicon PCR forward and reverse primers targeting the V3 and V4 regions of the 16S rRNA gene [32], followed by PCR cleanup with Agencourt Ampure XP (Beckman Coulter, Brea, CA, USA) magnetic beads, and index PCR for a second cleanup with magnetic beads. Normalization was based on the average size of the library as assessed with an Agilent High Sensitivity DNA Kit on a 2100 Bioanalyzer (Agilent Technologies, Santa Clara, CA, USA) and quantification with a NEBNext® Library Quant Kit for Illumina® (New England Biolabs, Ipswich, MA, USA) normalization. The normalized libraries were eventually pooled and loaded for sequencing on an Illumina MiSeq platform with paired-end 2 × 300 bp protocol using a MiSeq® Reagent Kit ver. 3 (600 cycles) (Illumina).

Neither blank controls nor mock communities were included in the present study; however, in order to limit the influence of contamination by extraction and amplification on the analysis, all samples were processed using the same DNA extraction reagents, and the amplifications were conducted with the same reagent lots.

Bioinformatic and statistical analysis

Reads were processed for quality filtering (using Q30 as threshold), adapter and primer removal BBDuk2 ver. 36.14; mate pairing was performed with BBMerge ver. 9.00 (https://sourceforge.net/projects/bbmap/). The fasta files were then processed using a Quantitative Insights Into Microbial Ecology (QIIME) 1.9.1 pipeline [33]. In detail, paired reads were merged in a single fasta file with multiple_split_libraries_fastq.py script, which provides further quality filtering. Operational taxonomic unit (OTU) picking was performed with the pick_open_reference_otus.py using the UCLUST method and with 97% identity to the Greengenes (version gg_13_8) reference database, followed by de novo clustering [34]. Representative sequences were checked for de novo chimera detection using ChimeraSlayer integrated in QIIME, and the chimeras were then filtered out from the OTU table [35]. The alpha and beta diversities were computed with the core_diversity_analyses.py script, rarefying the samples at 2500 reads. Samples with less than 2500 reads were excluded from the statistical analysis because these were not representative. Phyla, genera, and species abundance was reported as overall relative abundance, average relative abundance, and standard error of the mean (SEM).

Statistical support to the alpha diversity comparison between groups was assessed by nonparametric test with Monte Carlo permutations implemented in the compare_alpha_diversity.py script, while for the variance within and between groups, QIIME wrapper compare_categories.py was applied with permutational multivariate analysis of variance (PERMANOVA, Adonis method from R package Vegan implemented in QIIME). Statistically significant differences in OTU frequencies based on non-normalized raw counts between the NS and TTA samples from clinically healthy animals and those presenting at least one clinical sign suggestive of BRD were assessed using the differential_abundance.py script that implements the R package DESeq2 [36], and P values were adjusted (Padj) for multiple-testing with the false discovery rate (FDR) procedure of Benjamini and Hochberg [37]. OTUs were considered differentially abundant if at Padj ≤ 0.05 and if the estimated fold change was > 1.5 or < 1/1.5.

In order to evaluate the type I and type II errors and strengthen the results, we performed a power analysis on the data grouped by sample type, and by sample type and clinical signs according to the method presented by La Rosa and colleagues, implemented in the R package HMP, using the MC.Xmcupo.statistics function and 1000 Monte Carlo experiments [38].

Results

Study population

The number of calves selected from each farm ranged from 1 to 7, for a total of 22 calves (17 males and 5 females), aged from 5 to 14 months. Thirteen out of 22 animals (59%) were clinically healthy, and the remaining nine showed at least one clinical sign attributable to BRD (Table 1). Nasal swab samples were collected from 17 out of 22 animals, and TTA samples were collected from all animals. DNA was successfully extracted at a concentration above 5 ng/μl from 32 samples (13 NS and 19 TTA fluid samples). In one of the nine animals presenting clinical signs, the DNA concentration was below 5 ng/μl in both the NS and TTA samples; this animal was excluded from the study. At least one sample (NS or TTA) from 21 out of 22 calves was available for analysis. Further details regarding the study population are reported in Table 1.

Table 1 Data about calves (origin, signalment, history, clinical examination) and number of reads of each sample

Genetic analysis

After primer and quality trimming and pair merging, the total read count was 3,482,819, with an average read length of 407 ± 80 bp. After application of the multiple_split_libraries_fastq.py script to merge all the sequences in a single file, with further quality checks, the read number was 2,813,497. The total reads classified in the OTU table was 1,645,584, divided in 526,932 from the NS samples (median 24,072, min-max 159–167,198) and 1,118,652 from the TTA fluid samples (median 53,494, min-max 189–143,886). The number of assigned reads was below 2500 in 4 (2 NS and 2 TTA) out of 32 samples, and they were excluded from the analysis. Therefore, the final analysis was performed on 28 samples (11 NS and 17 TTA) from 19 calves (8 with clinical signs, 11 clinically healthy). Of these 28 samples, 18 (64.3%) were matched samples from the same animal (9 NS and 9 TTA) (Table 1). Finally, the reads obtained from these 28 samples were classified in 4368 OTUs (median 226.5, min-max 44–2502). The median (min-max) of the OTUs was 957 (495–2502) in the NS samples and 139 (44–719) in the TTA samples. A total of 810 unique sequences were classified as chimeric sequences and therefore removed from the OTU table before analysis.

Besides Mycoplasma, present in all samples, Delftia, Sphingomonas, and Agrobacterium composed the core biota of 90% of the samples. Twelve OTUs were present in all NS samples, including seven orders (Aeromonadales, Actinomycetales, Clostridiales, Flavobacteriales, Mycoplasmatales, Saprospirales, and Sphingomonadales) and four genera (Succinivibrio, Mycoplasma, Sphingomonas, and Corynebacterium). Overall, 123 out of 305 genera were found only in the NS samples and 16 genera only in the TTA samples (Additional file 2: Table S1).

Considering only the OTUs assigned at the species level, Pasteurella multocida (7.3% of total OTUs, 7.6% ± 3.7%) was the most abundant in the TTA fluid samples and Psychrobacter sanguinis (1.1% of total OTUs, 1.5% ± 0.6%) in the NS samples. The complete list of all species identified, when possible, is reported in Additional file 2: Table S2.

Comparison of bacterial composition between TTA fluid and NS samples

Alpha diversity values are reported in Table 2. Good’s coverage estimate with a rarefaction at 2500 was 91.6% ± 2.9% for the NS and 99% ± 0.9% for the TTA fluid samples. The alpha diversity indices and rarefaction curves of each sample are reported in Additional file 3.

There was a statistically significant difference in Shannon’s diversity index between the TTA fluids and the NS samples, considering the confidence interval. The microbial composition of the upper and lower respiratory tracts was compared by Bray-Curtis dissimilarity, weighted UniFrac, and unweighted UniFrac phylogenetic distances. The difference between the two bacterial communities was statistically significant as assessed by Adonis (P = 0.001), based on the three different distance matrices. Principal coordinates analysis (PCoA) plots of the methods are shown in Fig. 3. The type I error with a significance at 0.05 was < 0.001, as was the type II error, providing a power > 90%.

Fig. 3

Principal coordinates analysis (PCoA) 3D images. PCoA was performed using Bray-Curtis dissimilarity (a), unweighted UniFrac (b), and weighted UniFrac (c) distance matrices. Each sample is represented by a point with nasal swabs (NS = 11) in blue and trans-tracheal aspiration (TTA = 17) in red. The clustering observed between the NS and TTA samples indicates differences in the microbial compositions of these sampling sites

There were 741 OTUs with a statistically significant difference in abundance (as assessed by DESeq2 analysis) (details given in Additional file 4), with 19 more abundant in the TTA microbiota and 722 in the NS one.

Correlation of microbiota composition of NS and TTA fluid samples in relation to clinical status and farm of origin

Comparison of the microbiota composition of the TTA samples by farm of origin showed no statistically significant difference for this factor (Adonis on either Bray-Curtis dissimilarity, weighted UniFrac, or unweighted UniFrac distance; P > 0.05). It was not possible to estimate the type I and II errors because one group had size = 1. Similarly, no statistical difference in the microbiota composition of the NS samples was found when two statistical methods (Adonis on Bray-Curtis dissimilarity and weighted UniFrac distances; P > 0.05) were applied, except when compared based on unweighted UniFrac distance (P = 0.05). The type I error with a significance at 0.05 was < 0.001, as well as the type II error, providing a power > 90%. Finally, no correlation was found between the presence or absence of clinical signs and microbial composition of the NS and the TTA samples (Adonis on Bray-Curtis dissimilarity, weighted UniFrac, or unweighted UniFrac distance; P > 0.05, power > 90%).

Discussion

To the best of our knowledge, this is the first study using the 16S rRNA gene metabarcoding approach to characterize and compare the microbiota of the upper and lower respiratory tracts in calves with and without clinical signs of BRD. Recent studies have demonstrated the presence of several bacterial communities in the bovine nasopharynx, documenting that potential pathogenic bacteria are common inhabitants of the upper respiratory tract in cattle [25,26,27,28,29,30,31]. Our results are in agreement with the literature as regards the high number of phyla identified and the fact that five phyla seem to be dominant in the bovine upper respiratory tract microbiota: Proteobacteria, Tenericutes, Firmicutes, Actinobacteria, and Bacteroidetes [25, 26, 28,29,30,31].

Moreover, we found that the microbiota of the upper respiratory tract differs depending on the animals’ farm of origin. However, the number of calves was not equally distributed among the farms, and this difference was statistically significant based only on the unweighted UniFrac distance, which accounts for the presence/absence of observed OTUs. While it is difficult to draw general conclusions from the present data and further studies are needed to confirm this difference, it is reasonable to assume that environmental factors can influence, at least partially, nasal microbiota composition.

In fact, a variation in microbiota composition of the upper respiratory tract of calves when they are moved in a new environment has already been documented [26, 28]. Nevertheless, several factors have been observed to influence the development and composition of nasopharyngeal microbiota in humans (e.g., mode of birth delivery or breastfeeding) and possibly predispose to the development of respiratory disease [39, 40]. Moreover, differences in microbiota composition in relation to geographical provenience have also been found in humans [41].

A limitation to our study may be the absence of a blank control and a mock community, to calculate the PCR error rate and to evaluate the possible presence of contaminants in the process of DNA treatment. At the time of this study, the inclusion of sequencing controls was not a widespread practice and was not a part of similar studies [25, 26, 28].

Forty-five out of the 305 genera identified were possible contaminants, according to Salter et al. [42], but their relative abundance was low (Additional file 2: Table S1). Four of these genera were found with a relative abundance higher than 1% only in the NS samples: Sphingomonas, Delftia, Psychrobacter, and Corynebacterium. The relative abundance of contaminant genera was 0.6% in the TTA and 11.35% in the NS samples. As suggested by Salter et al. [42], since contaminant issues are more relevant in low biomass samples, it could be hypothesized that the bacterial load in the NS samples was lower, which would be odd, given that the upper airways are probably far more exposed to a higher environmental bacterial load [43]. A more probable explanation is that these genera were more abundant in the NS samples because of environmental contamination of the upper respiratory tract, rather than contamination occurring during the samples’ analysis due to low biomass.

Overall, the most abundant genus identified was Mycoplasma, which was abundantly found in all NS and TTA samples. This genus was previously identified with high abundance in the upper respiratory airways of both healthy and BRD-affected calves [26, 31]. Mycoplasma is spread worldwide, and it has frequently been isolated also with the use of bacterial culture and PCR detection from lower respiratory tract samples from calves, regardless of their clinical status [23, 24]. Unfortunately, in this study, the lack of information about Mycoplasma species present in the TTA samples precludes formulating a hypothesis about their pathogenetic role. Although M. bovis is recognized as a major etiologic agent in BRD and otitis media, less is known about other Mycoplasma spp., e.g., M. dispar and M. bovirhinis, which have been detected less frequently in the bovine respiratory tract [23, 24, 44,45,46,47]. It has been suggested that the lack of isolation of these two species could be correlated with an inhibitory effect of other mycoplasmas [24, 48]. Furthermore, discriminatory analyses within this genus could provide clues to determining the relationship between these species and their role in BRD.

Our observation of Moraxella, the second most abundant genus identified in the NS samples, is shared by Timsit et al. [26] and Lima et al. [31]. Lima et al. [31] also found a correlation between the presence of Moraxella and the development of BRD. In cattle, Moraxella bovis is the etiological agent of infectious bovine keratoconjunctivitis (IBK), and Moraxella genus has rarely been isolated in the course of BRD [49, 50]. In children, the role of this genus in the development of respiratory disease is controversial and is probably correlated with the species identified. In fact, it has been associated not only with the development of asthma and respiratory disease but also with a more stable microbiota, which is linked to a lower risk of developing respiratory disease [51,52,53]. Corynebacterium was identified in all NS samples, and previous studies have reported its relatively high abundance in the bovine upper respiratory tract [25, 26, 31]. In children, it has been correlated with a reduced risk of developing otitis media and respiratory disease [39, 54].

Four of the five most abundant phyla identified in the lower respiratory tract were the same as those found in the upper respiratory tract (Proteobacteria, Tenericutes, Actinobacteria, and Bacteroidetes), albeit with different abundance, though Fusobacteria seemed to be characteristic of this ecosystem. Identification of this phylum in the bovine upper respiratory tract has rarely been reported and each time with low abundance [25, 30, 31]. In other species, such as the dog and humans, Fusobacteria is one of the most abundant phyla found in the oral cavity but it is less abundant in the nasopharynx [43, 55, 56]. Furthermore, in the human lung, the abundance of Fusobacteria varies in relation to its presence in the oral cavity, leading to the hypothesis that the oral microbial community could be a bacterial source for lung microbiota composition [56,57,58,59,60].

The second most abundant genus identified in the TTA samples, and the main component of the phylum Proteobacteria, was Pasteurella. It was comprised mostly of P. multocida, and it was also identified with a lower abundance in the NS samples. In contrast, Pasteurellaceae were more abundant in oral than in lung and nasal samples from dog, and a higher abundance of Pasteurellales were found in the throat of sheep [43, 61]. P. multocida is considered a commensal of the upper respiratory airways, but its identification in samples from the lower respiratory tract has usually been correlated with BRD [22, 24]. Nevertheless, Angen et al. [23] isolated P. multocida from TTA samples obtained from clinically healthy animals. The absence of a significant difference in lower microbiota composition between healthy and BRD-affected calves suggests that P. multocida could be part of the microbial flora of the lower respiratory tract of healthy animals.

Our results showed significant differences in alpha diversity and beta diversity between the upper and the lower respiratory tract microbiota: the number of species composing the lower respiratory tract microbiota was lower, and these species differed by abundance and type from the upper respiratory tract microbiota. The same outcomes were obtained from studies in humans and dogs [3, 5, 60, 62]. In humans, the lung microbiota was found to differ significantly from the oral and the nasal microbiota [5, 62]. In healthy individuals, the lung microbiota partly overlaps with the oral microbiota [5, 62], which is the main source of the composition of the lung microbiota owing to the constant flow of saliva from the mouth, while much less liquid flows from the nose [60]. In upper respiratory tract disease, there is an increased liquid flow from the nose, with a higher potential to affect the lung microbiota as a consequence [60].

Analysis of respiratory tract samples obtained from the dog led to the hypothesis for a self-sustaining lung microbiota also in this species, which proved to be much more homogeneous than the composition of the oral or nasal microbiota [43]. In the present study, the trans-tracheal approach was used for the collection of samples from the lower respiratory tract in order to minimize the contamination from the upper respiratory ways. Moreover, this method has been recommended as optimal for evaluation of the microbiological status of the lower respiratory tract of calves [23]. The finding of 16 genera identified only in the lower respiratory tract, albeit few and with low abundance, suggests that the lung could be colonized by characteristic bacterial species also in cattle. Unfortunately, because of the paucity of information about the oral cavity microbiota of cattle, no conclusions can be drawn.

Comparison by farm of origin showed a statistical difference in microbiota composition only for the NS samples. This suggests that the lower respiratory tract microbiota may be more homogeneous and resilient than the upper respiratory tract, in agreement with the results found in the dog [43]. Moreover, these findings strengthen the hypothesis for a self-sustaining lower respiratory tract microbiota also in cattle.

The absence of significant differences in the bacterial species recovered from the NS and TTA samples from the healthy and the BRD-affected calves contrasts with previous results obtained in humans and cattle [7, 31]. Since BRD is a syndrome and not a single disease with a linear etiology, it may manifest clinically and microbiologically in several different forms [20]. Various other factors could have influenced our results and precluded differentiation between the microbiota of a diseased lung and that of a healthy one. Nevertheless, the primary aim of the present study was to characterize the microbiota of the respiratory airways of calves examined and sampled in field conditions.

Conclusions

Our findings demonstrate the presence of bacterial communities in the lower respiratory tract in both healthy calves and those presenting clinical signs of BRD. The results obtained from the NS samples suggest that environmental factors (farm, management) may influence the microbial composition of the bovine upper respiratory tract. The finding of bacterial communities in the lower respiratory tract, which differed from the ones found in the upper respiratory tract, suggests the presence of a self-sustaining microbiota at this level. Further studies including characterization of the oral cavity microbiota are needed to confirm this hypothesis.

Acknowledgements

The authors would like to thank the veterinary practitioners: Dr. Simona Ala, Dr. Simone Cabra, and Dr. Mauro Casalone for their cooperation and their willingness in referring the cases included in this study. Moreover, an acknowledgment goes also to the veterinary students that assisted the samples collection: Maurizio Beltramo, Giovanni Gallina, and Andrea Viglietti.

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Contributions

The project was conceived by CB. The following authors contributed to the study design and literature search: CB, IN, FC, SP, EG, ADA, and PG. The physical examination and samples’ collection was performed by CB and IN, with the help of IB. DNA extraction was performed by EG and IN. Library preparation, sequencing, and bioinformatic analysis were conducted by FC, with the help of IN. All authors contributed to the manuscript preparation and approved the final manuscript.

Corresponding author

Ethics declarations

Ethics approval and consent to participate

The study protocol was set up according to the ethical recommendations and approved by the animal care committee of the Department of Veterinary Sciences, University of Turin. The owners read and signed an informed owner consent form authorizing clinical procedures on their animals.

Consent for publication

Not applicable.

Competing interests

The authors declare that they have no competing interests.

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Alpha diversity metrics per sample. The alpha diversity metrics include Good’s coverage, Chao1 and observed species indices which estimate species richness, and Simpson and Shannon indices which estimate species evenness. (PDF 827 kb)

A table reporting the differential abundances of operational taxonomic units (OTUs) found in the nasal swabs (NS = 11) and in the trans-tracheal aspiration (TTA = 17) samples obtained by the DESeq2 analysis. As reported in the DESeq2 support information, the “base mean” column reports the mean of normalized counts for all samples, while the “log2FoldChange” column reports the log fold change calculated for the TTA as compared to the NS samples, with the relative standard error in the adjacent column “lfcSE” (that is log2 fold change standard error). For statistical significance, P values are reported without (P value) and with adjustment (Padj) for multiple testing with the false discovery rate (FDR). (XLS 1114 kb)

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